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Cosmids are plasmids that incorporate a segment of bacteriophage λ DNA that has the cohesive end site (cos) which contains elements required for packaging DNA into λ particles. Under apt origin of replication (ori), it can replicate as a plasmid.
In 1938, Craigie and Yen adapted Vi phages by selective propagation and used them at their critical test dilutions to differentiate 11 types of B. typhosus. [19] In 1943, Felix and Callow extended the method to Salmonella paratyphi B . in 1943 and differentiated 12 types with 11 phages. [ 20 ]
Cosmids are predominantly plasmids with a bacterial oriV, an antibiotic selection marker and a cloning site, but they carry one, or more recently two, cos sites derived from bacteriophage lambda. Depending on the particular aim of the experiment, broad host range cosmids, shuttle cosmids or 'mammalian' cosmids (linked to SV40 oriV and mammalian ...
The integration of phage λ takes place at a special attachment site in the bacterial and phage genomes, called att λ. The sequence of the bacterial att site is called attB, between the gal and bio operons, and consists of the parts B-O-B', whereas the complementary sequence in the circular phage genome is called attP and consists of the parts ...
The most often used are genes pIII or pVIII of bacteriophage M13. [5] The next step is the capturing step. It involves conjugating the phage library to the desired target. This procedure is termed panning. It utilizes the binding interactions so that only specific peptides presented by bacteriophage are bound to the target.
Embark was founded in Austin, Texas, in 2015 by brothers Adam Boyko and Ryan Boyko, Matt Salzberg, and Spencer Wells. [1] [2] Prior to the formation of the company, the Boyko brothers spent nearly a decade collecting thousands of DNA samples from dogs for research into the origin of dogs and what DNA can reveal about their health.
MS2 tagging is a technique based upon the natural interaction of the MS2 bacteriophage coat protein with a stem-loop structure from the phage genome, [1] which is used for biochemical purification of RNA-protein complexes and partnered to GFP for detection of RNA in living cells. [2]
The simplest DNA end of a double stranded molecule is called a blunt end. Blunt ends are also known as non-cohesive ends. In a blunt-ended molecule, both strands terminate in a base pair. Blunt ends are not always desired in biotechnology since when using a DNA ligase to join two molecules into one, the yield is significantly lower with blunt ...